Method and Materials for Quaternary Amine Catalyzed Bisulfite Conversion of Cytosine to Uracil

United States Patent Application 20100087641

Kind
Code:

A1

Abstract:

The invention provides methods and materials for the conversion of cytosine to uracil. A nucleic acid, such a gDNA, is reacted with bisulfate, such as magnesium bisulfite, in the presence of a quaternary amine catalyst. Examples of suitable quaternary amine catalysts include but are not limited to quaternary ammonium compounds, quaternary alkyl ammonium salts, quaternary alkyl ammonium halides, quaternary methyl ammonium bromide, quaternary ammonium chloride, tetraethyl ammonium hydroxide, tetraethylammonium chloride, tetrabutyl ammonium chloride, tetrabutyl ammonium bromide. The invention also contemplates kits of premeasured ingredients for carrying out the methods of the invention either on an individual sample or on a plurality of samples.

1. A method for converting cytosine to uracil comprising the steps of: providing a nucleic acid comprising at least one cytosine nucleobase; and reacting the nucleic acid with a bisulfite ion, in the presence of a quaternary amine catalyst having the Formula: or a derivative thereof, wherein: R1, R2, R3 and R4 are each independently C1-C4 alkyl; and Z is selected from halides and OH.

2. The method of claim 1, wherein the nucleic acid is gDNA and further wherein a step of predenaturation of the gDNA prior to the step of reacting the gDNA with the bisulfite ion is not performed.

16. The kit of claim 15 wherein the tetraethyl ammonium hydroxide is provided as an approximately 20% solution.

17. The kit of claim 12 further comprising NaOH, wherein the NaOH is provided as an approximately 0.1M solution.

18. The kit of claim 12 further comprising a nucleotide polymerase and one or more primers for sequencing or amplification.

19. The kit of claim 12 further comprising one or more reaction vessels.

20. The kit of claim 12 further comprising prepackaged materials sufficient to convert cytosine to uracil in one or more nucleic acid samples containing at least one cytosine nucleobase.

Description:

This application is a continuation of application Ser. No. 10/926,528, filed Aug. 26, 2004 and claims benefit of priority to U.S. Provisional Application Ser. Nos. 60/499,106 filed Aug. 29, 2003 and 60/523,054 filed Nov. 17, 2003, each of which is hereby incorporated by reference.

FIELD

The invention relates generally to methods and materials for the conversion of cytosine to uracil.

BACKGROUND

Assessment of methylation of DNA is useful in many research, diagnostic, medical, forensic, and industrial fields. Key to this assessment is converting cytosine, but not methylcytosine, to uracil, but not thymine. One basic method for such conversion, employing sodium bisulfite, is well known. Over the years, the method has been improved in attempts to overcome disadvantages that include tedious procedures, lengthy reaction times, and DNA degradation. The most commonly used protocol is taught by J. Herman, Proc. Natl. Acad. Sci. 93, 9821-26 (1996), incorporated herein by reference in its entirety. This method involves denaturation, reaction with sodium bisulfite in the presence of hydroquinone, and subsequent completion of the modification by treatment with NaOH. Despite the attempts to improve the protocol, current procedures require pre-denaturation of the genomic DNA (gDNA) to single stranded DNA (ssDNA), preparation of fresh solutions of sodium bisulfite (NaHSO3), typically about 3M, and inclusion of an anti-oxidant (e.g., hydroquinone). The protocol also requires long reaction times and tedious clean-up procedures.

In addition, the currently employed sodium bisulfite protocols are plagued by reports of incomplete conversion, irreproducible results, and other problems. In some cases, the reaction can result in significant DNA degradation (reportedly as high as 96%), making it difficult to obtain enough sample for further analysis. See. S. J. Clark et al. Nucleic Acid Research 2001, 29 no. 13, e65. Given the importance of assessment of DNA methylation, it can be seen that there is a need for improved methodologies for conversion of cytosine to uracil.

It has been discovered that bisulfite methods that employ magnesium bisulfite, polyamine compounds, and/or quaternary amine compounds provide useful alternatives to sodium bisulfite conversion reactions. These discoveries are the subjects of co-owned applications entitled “Method And Materials For Polyamine Catalyzed Bisulfite Conversion Of Cytosine To Uracil” (U.S. application Ser. No. 60/499,113 filed Aug. 29, 2003, and also application Ser. No. 60/499,113 (docket no. 5065P2) having the same title and filed Nov. 17, 2003), “Method And Materials For Quaternary Amine Catalyzed Bisulfite Conversion Of Cytosine To Uracil” (U.S. application Ser. No. 60/499,106 filed Aug. 29, 2003, and “Method and Materials for Bisulfite Conversion of Cytosine to Uracil” (U.S. application Ser. No. 60/499,082 filed Aug. 29, 2003, and also application Ser. No. 60/523,056 having the same title and filed Nov. 17, 2003), all of which are hereby incorporated by reference in their entirety Improvements in clean-up procedures associated with conversion of cytosine to uracil are also the subject of co-owned applications entitled “Improved Bisulfite Method” (U.S. application Ser. No. 60/498,996 filed Aug. 29, 2003, and also application Ser. No. 60/520,941 (5109P2) having the same title and filed Nov. 17, 2003) all of which are hereby incorporated by reference in their entirety.

SUMMARY

In certain embodiments of the invention, the invention comprises methods of specifically converting cytosine to uracil by using a catalyzed bisulfite reaction.

In some embodiments, the present invention provides methods for the conversion of cytosine to uracil in a nucleic acid comprising the steps of:

reacting a nucleic acid comprising at least one cytosine nucleobase with bisulfite ion in the presence of a quaternary amine catalyst.

In some embodiments, the quaternary amine comprises a compound having Formula I:

or a derivative thereof, wherein:

R1, R2, R3 and R4 are each independently alkyl, preferably C1-C4 alkyl; and

Zθ is selected from the halides and OFF.

In some embodiments, R1, R2, R3 and R4 are identical.

In some embodiments of the invention, the quaternary amine catalyst comprises a quaternary ammonium compound, or a derivative thereof. In further embodiments, the quaternary amine catalyst comprises a quaternary alkyl ammonium salt. In yet further embodiments, the quaternary amine catalyst comprises a quaternary alkyl ammonium halide, for example a quaternary ammonium chloride or a quaternary ammonium bromide. In some embodiments, the quaternary amine catalyst comprises at least one of quaternary methyl ammonium bromide, tetraethyl ammonium hydroxide, tetraethylammonium chloride, tetrabutyl ammonium chloride and tetrabutyl ammonium bromide.

In some embodiments, the reaction of the nucleic acid and bisulfite ion is performed in a solution containing bisulfite ion, such as magnesium bisulfite, in a concentration of from about 0.5M to about 2.5M. In further embodiments, the solution contains bisulfite ion, such as magnesium bisulfite, in a concentration of from about 1M to about 2M.

In some embodiments, the magnesium bisulfite is present at a concentration of at least about 1M.

Also provided are methods for the conversion of cytosine to uracil comprising the steps of reacting a DNA sample in solution with a bisulfite salt and quaternary amine catalyst as described above, wherein the concentration of the bisulfite salt is from about 0.5M to about 2M. In further embodiments, the concentration of the bisulfite salt is about 1.3M.

In some embodiments of the methods of the invention, the reaction is performed at a temperature from about 40 to about 60 degrees, such as about 50 degrees, for about 4 to about 15 hours. In further embodiments of the methods of the invention, the nucleic acid is gDNA.

Also provided in accordance with the present invention are kits for use in conversion of cytosine to uracil comprising magnesium bisulfite; and a quaternary amine catalyst as described above. In some embodiments of such kits, the magnesium bisulfite is provided as an approximately 2M magnesium bisulfite solution. In further embodiments of the kits of the invention, the quaternary amine catalyst comprises tetraethyl ammonium hydroxide. In some embodiments, the kits further comprise reagents for sequencing and/or amplification (e.g., by PCR), for example a polymerase and one or more primers. In some embodiments, the kits contain premeasured materials useful in various embodiments of the methods of the invention.

In some embodiments, the methylation status of one or more cytosines in the target nucleic acid(s) can be determined by any suitable method. Typically, methylation status can be determined by measuring the presence or relative amount of uracil at a nucleotide position that was previously non-methylated cytosine, and was converted to uracil by the bisulfite treatment. If desired, the presence or relative amount of residual cytosine at the same nucleotide position (indicating the presence of methylcytosine) can be measured for comparison with the amount of uracil, to determine the degree of methylation at the particular nucleotide position. Appropriate control experiments can also be performed to correct for incomplete transformation of cytosine to uracil, if desired.

The presence or amount of uracil and/or methylcytosine at a particular nucleotide position can be measured by any suitable method, such as DNA sequencing (e.g., by the Sanger method or Maxam-Gilbert method or subsequent embodiments thereof (e.g., using dye-labeled terminators or dye-labeled primers, such as discussed in WO 02/30944 and by Ansorge et al. DNA Sequencing Strategies—Automated and Advanced Approaches, John Wiley & Sons, New York, 1997)), PCR (e.g., primer-specific PCR), oligonucleotide ligation assay (OLA) or other ligation-dependent techniques (e.g., see U.S. Pat. No. 6,511,810 and references cited therein), single base extension (over the potential methylation site), mass spectrometry, real time PCR (e.g., using labeled probes that are complementary to C and or U), microarrays comprising sequence specific probes, etc. Various exemplary techniques are also described by Kirk et al., Nucl. Acids Res., 30:3295-3311 (2002).

DETAILED DESCRIPTION

It is to be understood that both the foregoing general description and the following detailed description are exemplary and explanatory only and are not restrictive of the invention, as claimed. In this application, the use of the singular includes the plural unless specifically stated otherwise. In this application, the use of “or” means “and/or” unless stated otherwise. Furthermore, the use of the term “including”, as well as other forms, such as “includes” and “included”, is not limiting. Also, terms such as “element” or “component” encompass both elements and components comprising one unit and elements and components that comprise more than one subunit unless specifically stated otherwise.

The section headings used herein are for organizational purposes only and are not to be construed as limiting the subject matter described. All documents, or portions of documents, cited in this application, including but not limited to patents, patent applications, articles, books, and treatises, are hereby expressly incorporated by reference in their entirety for any purpose.

As used herein, the term “EXO/SAP” denotes a mixture of exonuclease I (EXO) and shrimp alkaline phosphatase (SAP).

As used herein, the term “gDNA” refers to genomic DNA.

Bisulfite ion has its accustomed meaning of HSO3−. Typically, bisulfite is used as an aqueous solution of a bisulfite salt, for example magnesium bisulfite, which has the formula Mg(HSO3)2, and sodium bisulfite, which has the formula NaHSO3.

The term “PCR” is intended to denote polymerase chain reaction, as is well known in the art. The term “MSP” denotes methylation specific PCR, such as described by J. Herman, Proc. Natl. Acad. Sci. 93, 9821-26 (1996), and modified as discussed herein.

As used herein, the term “nucleic acid” includes, for example, nucleobase-containing polymeric compounds, including naturally occurring and non-naturally occurring forms thereof, for example and without limitation, genomic DNA, cDNA, hnRNA, mRNA, rRNA, tRNA, fragmented nucleic acids, nucleic acids obtained from subcellular organelles such as mitochondria or chloroplasts, and nucleic acids obtained from microorganisms, or DNA or RNA viruses that may be present on or in a biological sample.

All reported temperatures are in degrees Celsius unless stated otherwise.

In some embodiments, the present invention provides methods of converting cytosine to uracil in a nucleic acid sample by using a catalyzed bisulfite reaction. The methods of the present invention can provide significant benefits.

The nucleic acid samples may be obtained by any conventional collection and purification process prior to use in the methods of the invention. The examples discussed below used commercially available sample lines (e.g. from Coriell or Intergen) of known methylation status, to assess the viability of the methods.

Typically, the product of the reaction between the nucleic acid and bisulfite is reacted with a base to complete the conversion of cytosine to uracil. One typical base is NaOH. In some embodiments the methods herein further comprise the step of purifying the bisulfite-reacted nucleic acid prior to treatment with base. In some further embodiments, the methods further comprise the step of analyzing the product of the bisulfite conversion reaction, for example by mass spectrometry, to confirm completion of the bisulfite conversion reaction.

Typical protocols in the art require the use of 3M sodium bisulfite, long reaction times of up to 16 hours, and the presence of an antioxidant. Because of the relatively high salt concentration, the low pH of the reaction and the long reaction times, the DNA can be degraded. Additionally, the ss DNA resulting from the gDNA is difficult to purify away from the high salt concentration used in the reaction. In addition, it is typically necessary to remove most of the bisulfite, which interferes with subsequent enzymatic reactions, for example those of PCR protocols. Prior procedures also require freshly prepared solutions of bisulfite and antioxidant (typically hydroquinone).

Embodiments of the methods of the present invention may overcome one or more disadvantages of prior methods. For example, it has been discovered in accordance with the some embodiments of the present invention that the reaction of a nucleic acid of interest with bisulfite ion, such as magnesium bisulfite, in the presence of a quaternary amine in accordance with the methods disclosed herein afford faster reaction times. In addition, because the reaction time is faster, less oxidation may occur. Thus, the presently disclosed methods do not require addition of an antioxidant such as hydroquinone. Additionally, magnesium bisulfite solution at 1M concentration may remain acidic in the presence of effective concentrations of polyamine catalyst (for example 0.1M DETA), whereas the corresponding solution of sodium bisulfite salt does not. Thus, methods of the invention can employ bisulfite concentrations that are significantly less than the methods known in the art, thereby affording facilitated sample preparation for PCR. Moreover, it has been discovered herein that stock magnesium bisulfite solutions can be employed, thus eliminating the need to freshly prepare those solutions. Finally, methods of the invention reduce or eliminate the need for a separate predenaturation step, and can be performed in a greatly reduced reaction volume. Thus, methods of the present invention can afford PCR yields similar to those of protocols previously known in the art, but with reduced preparation times, reaction times, and clean-up efforts.

In certain embodiments, the invention comprises kits for carrying out the methods of the invention. In one embodiment, a kit of the invention includes pre-measured ingredients required for carrying out the bisulfite reaction, such as magnesium bisulfite and catalyst. In certain embodiments, the catalyst comprises tetraethyl ammonium hydroxide. In certain embodiments, the invention includes a kit containing pre-packaged materials sufficient to prepare multiple samples. In yet another embodiment, the materials will be pre-packaged with appropriate Eppendorf tubes or other reaction vessels, as appropriate.

The section headings used herein are for organizational purposes only and are not to be construed as limiting the subject matter described. All documents, or portions of documents, cited in this application, including but not limited to patents, patent applications, articles, books, and treatises, are hereby expressly incorporated by reference in their entirety for any purpose.

The examples described herein are certain embodiments chosen to illustrate the invention. Applicant does not limit the invention to these embodiments. Rather, Applicant acknowledges that those reasonably skilled in the art will readily recognize additional variants that do not differ from the scope and spirit of the inventions disclosed herein.

EXAMPLES

In accordance with the present invention, it has been found that quaternary amines, such as tetraethylammonium hydroxide (ET4NOH), are useful catalysts in the bisulfite conversion of cytosine to uracil in nucleic acid samples.

Methyl-Specific PCR Analysis

Each sample discussed herein was analyzed by methyl-specific PCR (MSP). MSP provides a relatively fast analysis method for methylation status of bisulfite-treated DNA samples, providing a yes/no answer. The method is based on using primer pair sets. One primer pair is designed to anneal/PCR amplify only if all cytosines were successfully converted to uracil, and the other primer pair in the set annealed/PCR amplified if the methylated cytosine (CpG cytosines only) were methylated, and therefore not converted to uracil.

The MSP pairs that amplify specific gene fragments, and the expected size of the amplicon, are the following:

for the p16 gene, unmethylated reaction (size 151):

5′-TTATTAGAGGGTGGGGTGGATTGT-3′

(sense),

5′-CAACCCCAAACCACAACCATAA-3′

(antisense);

methylated reaction (size 150):

5′-TTATTAGAGGGTGGGGCGGATCGC-3′

(sense),

5′-GACCCCGAACCG-CGACCGTAA-3′

(antisense);

for the MGMT gene, unmethylated reaction (93):

5′-TTTGTGTTTTGATGTTTGTAGGTTTTTGT-3′

(sense),

5′-AACTCCACACTCTTCCAAAAACAAAACA-3′

(antisense);

methylated reaction (81):

5′-TTTCGACGTTCGTAGGTTTTCGC-3′

(sense),

5′-GCACTCTTCCGAAA-ACGAAACG-3′

(antisense);

for the DAP-kinase gene, unmethylated reaction:

5′-GGAGGATAGTTGGATTGAGTTAATGTT-3′

(sense),

5′-CAATCCCT-CCCAAACACCAA-3′

(antisense);

methylated reaction:

5′-GGATAGTCGGATCGAGTTAACGTC-3′

(sense),

5′-CCCTCCCAAACGCCG-3′

(antisense);

for the MLH1 gene, unmethylated reaction (124):

5′-TTTTGATGTAGATGTTTTATTAGGGTTGT

(sense)

5′-ACCACCTCATCATAACTACCCACA

(antisense)

methylated reaction (115)

5′-ACGTAGACGTTTTATTAGGGTCGC

(sense)

5′-CCTCATCGTAACTACCCGCG

(antisense)

for the p15 gene, unmethylated reaction (154):

5′-TGTGATGTGTTTGTATTTTGTGGTT

(sense)

5′-CCATACAATAACCAAACAACCAA

(antisense)

methylated reaction (148)

5′-GCGTTCGTATTTTGCGGTT

(sense)

5′-CGTACAATAACCGAACGACCGA

(antisense)

The PCR recipe used to evaluate the samples was:

2X Taq Gold PCR Master Mix

10 μL

Fwd primer (5 μM)

1 μL

Rev primer (5 μM)

1 μL

Bisulfite treated DNA

0.5 μL

H2O

7.5 μL

20 μL

2×TaqGold PCR master mix is commercially available from Applied Biosystems. The forward and reverse primer sequences are those listed above.

The following thermal cycling schedule was used:

40 cycles

95 deg 5 min

95 deg 30 sec

60 deg 45 sec

72 deg 1:00 min

4 deg forever

One of the primers in each set was synthesized with a 5′FAM label. A 1 uL aliquot of the above PCR reaction was added to HiDi formamide with ROX 500 size standard added, and denatured by heating at 95° C. for 5 min By using a FAM-labeled primer, the PCR amplicon was directly analyzed on an ABI PRISM® 310 Genetic Analyzer, with POP-4™ polymer, using run module “GS POP4 (1 μL) A” (reagents and instrument all from Applied Biosystems).

The presence of a PCR amplicon (i.e. a “peak”) having the correct size as observed using the 310 Genetic Analyzer indicated a successful reaction. Additionally, the height or area of the peak could be used empirically to determine how much template (i.e. bisulfite-treated gDNA) was initially present. The bigger the peak, the more DNA was initially present.

The MSP-PCR product was then sometimes sequenced for further “resolution”. DNA sequencing was by standard protocol and reagents from Applied Biosystems.

Prior to sequencing of the PCR amplicon, the primers and excess dNTPs used during the MSP-PCR were removed by treatment of a 4 μL aliquot of the PCR reaction with an equal volume mixture containing 2 Units each of Shrimp Alkaline Phosphatase (SAP) and exonuclease 1 (exo) (USB Corporation, Cleveland, Ohio). The reaction was incubated at 37° C. for 1 hr, and then heat-denatured at 75° C. for 15 min. A 4 μL aliquot of the exo/SAP reaction was added to a solution containing 1-4 μL of BigDye® Terminator v1.1 cycle sequencing reaction mix (Applied Biosystems), 2 μL of BigDye® Terminator v1.1 5× sequencing buffer, 2 μL of the reverse PCR primer (5 μM) (which did not have a FAM-label), and enough water for a final volume of 20 μL. Thermal cycling: 95° C./1 min, 50 cycles of 96° C./10 sec, 52° C./10 sec, 60° C./4 min, and stored at 4° C. The cycle-sequencing reaction products were purified by an Edge Biosystems Performa® 96-well plate, dried under vacuum, dissolved in 20 μL of HiDi Formamide and analyzed on an ABI Prism 3730 DNA Analyzer with KB basecaller or a 3700 DNA Analyzer.

General Protocol for Quaternary Amine Conversion

A basic protocol for the quaternary amine conversion reaction is set forth below for purposes of illustration. In an Eppendorf tube, or other suitable vessel, about 300 ng DNA, 10 μL water, 10 μL 20% Et4NOH (to about 0.1 mM final concentration), and 85 μL magnesium bisulfite (to about 1.3M final concentration) are combined. The resulting mixture is incubated at about 50° for 4 to 15 hours, prior to purification and subsequent PCR of the treated product. Purification can be conducted by existing means, such as in accordance with the protocol of J. Herman, DNAs 93, 9821-26 (1996), incorporated herein by reference in its entirety, or with commercially available kits such as the Wizard DNA clean-up kit (available from Promega) or the EZ DNA Methylation Kit™ (available from Zymo Research).

A new purification method, which recovers the bisulfite-treated DNA very effectively, is the subject of the application entitled “Improved Bisulfite Method” (U.S. application Ser. No. 60/498,996 filed Aug. 29, 2003, and also application Ser. No. 60/520,941 (5109P2) having the same title and filed concurrently herewith) each of which is hereby incorporated by reference in its entirety.

In contrast with known sodium bisulfite conversion reaction protocols, all bisulfite conversion reactions disclosed herein were carried out without predenaturation, and without the inclusion of an antioxidant (e.g., hydroquinone), unless otherwise indicated.

The magnesium bisulfite used in the Examples described herein was purchased as a 2M Mg (HSO3)2 solution from Aldrich Chemical Co., Milwaukee, Wis. The pH of the solution was 2.6. The solution was used off-the-shelf, as purchased, and was not freshly prepared prior to each use.

The resultant products were purified by standard methods (Wizard kit) and analyzed by MSP using the following MSP primer set: p15M, Dapk M, MgMt M, and p16M and four corresponding unmethylated templates: p15 U, Dapk U, MgMt U, and p16 U. The methylated primer pairs, p15M, Dupk M, Mgmt M, and p16M were all negative, as expected, since the gDNA sample was not expected to be methylated. No product peak was expected or seen as with the p15M template. However, for the unmethylated gDNA samples, well-defined product peaks were seen in Et4NOH and TBAC catalyzed reactions when the unmethylated primer pairs were used in MSP analysis.

Effect of Antioxidant and Concentration of Quaternary Amine

Examples 5-8, shown below in Table 2, vary with respect to the presence or absence of antioxidant, and the identity and amount of quaternary amine.

TABLE 2

Ex. 5

Ex. 6

Ex. 7

Ex. 8

3 μL NA 13705

3 μL NA 13705

3 μL NA 13705

3 μL NA 13705

5.5 μL 2M NaOH

5.5 μL 2M NaOH

35 μL water

35 μL water

45 μL 2M TBAC

45 μL 2M TBAC

10 μL 20% Et4NOH

20 μL 20% Et4NOH

incubate at 37° for 10-12

incubate at 37° for 10-12

minutes

minutes

55 μL 2M Mg(HSO3)2

30 μL Hydroquinone

85 μL 2M Mg(HSO3)2

60 μL 2M Mg(HSO3)2

—

85 μL 2M Mg(HSO3)2

—

—

Each of Examples 5-8 were incubated at 50° for four hours. The reaction mixture in example 8 immediately formed a large amount of precipitate, which remained even after incubation, and was excluded from further study. Example 7 had a non-interfering amount of precipitate and was retained in the study. After the four hour incubation, the remaining three samples were purified according to the new purification method referred to above, which employed a size-exclusion purification process. The process uses a Microcon 100 (Millipore) size-exclusion device. The sample and 200 μL of water were added to the Microcon 100 device, and the sample was then spun in the device at approximately 2800 RPM for about 8 minutes (as per manufacturers recommendation). The resultant filtrate was removed. Two subsequent washes with about 300 μL water, each spun at about 2800 RPM for 8 minutes followed. After each, the filtrate was again removed. About 300 μL 0.1N NaOH was added and spun at approximately 2800 RPM for about 8 minutes. Again, the filtrate was removed. After addition of about 300 μL of water, the sample was spun in the device at 2800 RPM for about 6-8 minutes. The filtrate was removed and about 50 μL TE buffer (approximately pH 8) was added. After about 5 minutes before it was inverted to collect the purified DNA sample in a centrifuge. Approximately 60 μL were collected.

The bisulfite-treated DNA was analyzed by MSP using the following MSP primer sets: p15 M, p15 U, Dapk M, Dapk U, Mgmt M, Mgmt U, p16 M, and p16 U. Hydroquinone did not appear to greatly enhance PCR yields. The Et4NOH sample displayed a far greater product peak than TBAC with or without hydroquinone. Only about 6 ng of bisulfite-treated gDNA was used per PCR. Prior experiments using the published purification protocol (Wizard resin) provided much less isolated DNA based on the amount required for successful PCR. These data support the use of quaternary amine, and specifically Et4NOH, as a catalyst.

The samples in Examples 9-12, shown in Table 3, demonstrate the bisulfite conversion of reduced amounts of DNA. These samples vary with respect to either the amount of DNA used, or reduced concentration of magnesium bisulfite/Et4NOH.

TABLE 3

Ex. 9

Ex. 10

Ex. 11

Ex. 12

3 μL Coriell 13705

1 μL Coriell 13705

1 μL Coriell 13705

1 μL Coriell 13705

35 μL water

35 μL water

35 μL water

35 μL water

10 μL 20% Et4NOH

10 μL 20% Et4NOH

5 μL 20% Et4NOH

2.5 μL 20% Et4NOH

85 μL 2M Mg(HSO3)2

85 μL 2M Mg(HSO3)2

40 μL 2M Mg(HSO3)2

85 μL 2M Mg(HSO3)2

~1.3M final

~1.3M final

~1.0M final

~0.8M final

Example 9 (34, of Coriell) contained about 1 μg DNA, and Examples 10-12 (1 μL of Coriell) contains about 300 ng DNA. Each of these samples was allowed to react as previously discussed, at 50° C. for four hours. Subsequent to this incubation period, each was subject to the size-exclusion purification process discussed above, using the Microcon 100 device. The process differed from that previously discussed only in that slightly more water was used, and about 350 μL of 0.1M NaOH was used. Each was collected in about 504, TE buffer, and 14, was used in subsequent PCR. Surprisingly, the 300 ng sample at 1.3M magnesium bisulfite (Example 10) was observed to provide more PCR product than the 1 μg sample (Example 9).

Effect of Enzyme Concentration and Template (gDNA) Concentration in MSP

The same bisulfite-treated samples above, specifically, Ex. 9 and Ex. 10, were further analyzed by MSP under alternative conditions: (a) additional polymerase (TaqGold) and (b) less bisulfite-treated gDNA template. The MSP conditions are shown in Table 4, below.

TABLE 4

Ex. 13

Ex. 14

Ex. 15

Ex. 16

Ex. 17

Ex. 18

Ex. 9

Ex. 10

NTC

1/10 of

1/20 of Ex. 9

1/30 of Ex. 9

bisulfite-

bisulfite-

with xs

Ex. 9

bisulfite-

bisulfite-

treated

treated

enzyme

bisulfite-

treated DNA

treated DNA

DNA

DNA

treated

(0.3 ng/μL)

(0.2 ng/μL)

with xs

with xs

DNA

enzyme

enzyme

(0.6 ng/

μL)

Each PCR was prepared as described in the MSP analysis described elsewhere herein. MSP primer sets used were Mlh M, Mlh U, Dapk M, Dapk U, Mgmt M, Mgmt U, p16 M, and p16 U. When excess TaqGold polymerase was used, an additional 24, (2 units) was added to the reaction.

The results show that extra enzyme in the Master Mix forced “mispriming” to occur (determined by subsequent sequencing). The 1/10, 1/20, and 1/30 dilutions of the Microcon 100 purified bisulfite-treated gDNA still provided enough gDNA template for MSP for almost all of the reactions. Successful PCR was seen even when only 0.2 ng of gDNA was used in MSP. Although there were two data points that “dropped out,” overall the data are excellent. Thus, it appears that as little as 0.2 ng of DNA can be used with successful PCR yields.

Studies Using Additional Templates

The studies above included only unmethylated DNA. The following experiments include side by side comparisons of methylated to unmethylated gDNA. Five additional “control” reactions were evaluated with both methylated and unmethylated gDNA. These samples contained 1 μL DNA from Coriell or 3 μL DNA from the Intergen p16 kit (each about 300 ng DNA), 35 μL water, 104, 20% Et4NOH, and 854, 2M magnesium bisulfite and heated at 50° C. for about 4 hours. The samples were Coriell #34 and #35, and DNA from Intergen's p16 “kit,” p16U, p16M, and a universally methylated gDNA. Each was incubated at 50° for four hours and subjected to the size-exclusion clean-up method, using a Microcon 100 filtration unit received 50 μL TE. One μL was used in MSP with the following MSP primer pairs: MLH M, MLH U, Dapk M, Dapk U, Mgmt M, Mgmt U, p16M, and p16 U. Excellent MSP yields were obtained as evidence by an amplicon of the correct size, several of the PCRs were subjected to direct sequencing.

The same bisulfite treated samples were additionally analyzed by sequencing with other primers for different gene targets: E2F2, Frap, Xpd, CDKN1C, Ral GDS, Etsl, Cdhl, Apcl, Esrl, MLh1, and CMyc. These primers are:

E2F2FwdFam

FAM-GGTTTGGGGAATATATTGTTGGG

E2F2Rev

CTTAAAAAAACAACCACACCTACTATTAATACC

Cdh1FwdFam

FAM-TGTGTTTGTAGGAGTTTGTGTTTGTG

Cdh1Rev

CTCCAAAATCCTCCAAACCC

Frap1FwdFam

FAM-GATTGGTTTTTAGGGTTGGGAA

Frap1Rev

TCCCCTAACCCCCCCTC

XpdFwdFam

FAM-GGGTTTGATTAATATTTAATTTTGGTAGG

XpdRev

TCAATCCACTAAAACACAACCAATC

CDKN1CfwdFam

FAM-GTTTTATAGGTTAAGTGTGTTGTGTT

CDKN1Crev

CACTAATACTAAAAAAATCCCACAAAC

RalGDSFwdFam

FAM-GGGTTTTATAGTTTTTGTATTTAGGTTTTTATTG

RalGDSRev

CAACTCAATAAACTCAAACTCCCC

ID2FwdFam

FAM-GAAGGTGAGTAAGATGGAAATTTTGTAGTA

ID2Rev

ACTAACAATTTCACACACAACTCAATCTAC

ApclFwdFam

FAM-AGGGAAAATTGGAGTAGGAGGTT

ApclRev

ACTCAACTCCCCAAAACTATCCTTAA

Esr1FwdFam

FAM-TGGGAGATTAGTATTTAAAGTTGGAGG

Esr1Rev

CCTTAAATCTAATACAATAAAACCATCCC

Ets1FwdFam

FAM-GGGAATTTGAGATTTTTGGGAAG

Ets1Rev

CCCAACTACCAACAACATCCC

Mlh1FwdFam

FAM-GTAGTTTTTTTTTTAGGAGTGAAGGAGGT

Mlh1Rev

CCCTACTCTTATAACCTCCCACAAAT

CMycFwdFam

FAM-GGGAGGTTATTTTGTTTATTTGGG

CMycRev

CCAAAACCCAAAAAACAATTAACAC

Comparison of Magnesium Bisulfite/Et4NOH to Sodium Bisulfite Protocol After 6 Hour and 15 Hour Reaction Times

A direct comparison between samples prepared according to the sodium bisulfite protocol (J. Herman, Proc. Natl. Acad. Sci. 93, 9821-26 (1996)) and the magnesium bisulfite protocol as described in Ex. 10 was conducted, using Et4NOH, NaOH, and no additive. Two plates were set up, one for a 6 hour analysis and the other for a 15 hour analysis. Both reactions took place at 50° C. Only an unmethylated gDNA sample was investigated. All reaction products were purified by the size-exclusion clean-up procedure described above and recovered in a final volume of 504, of TE MSP was used to analyze the converted DNA. The sodium bisulfite procedure provided gDNA that gave excellent results in MSP. The magnesium bisulfite converted gDNA gave much weaker signals in MSP than the sodium bisulfite converted DNA. However, the magnesium bisulfite/Et4NOH differs from the sodium bisulfite protocol in significant ways. The magnesium bisulfite/Et4NOH was achieved without a pre-denaturation step, much lower concentration of bisulfite, no exacting pH control, no antioxidant, and reagents were “off the shelf” and not freshly prepared.

The size-exclusion purification worked well on the sodium bisulfite samples as well as the magnesium bisulfite samples.

Direct Comparison of Magnesium Bisulfite with Et4NOH and Sodium Bisulfite Reactions on Both Methylated and Unmethylated gDNA

The 1.3M (final concentration) magnesium bisulfite with Et4NOH reaction was compared to the samples treated with sodium bisulfate, according to the known method. The magnesium bisulfite recipe was 1 μL Coriell or 3 μL Intergen, 32 or 34 μL water, 10 μL 20% Et4NOH, 85 μL 2M magnesium bisulfite. Two methylated samples and two unmethylated samples were compared in side by side reactions with sodium bisulfite and the magnesium bisulfite. These were allowed to react for 6 and 15 hours at 50° for a total of sixteen (16) samples processed. Purification by the size-exclusion process described above was performed. In this very thorough comparison, the 16 samples, purified by Microcon 100, were all analyzed by sequencing. (The sequencing analysis allows for all cytosine in a given region to be analyzed for completeness of the bisulfite conversion to uracil.)

Eleven different primer sets for specific gene targets were used: E2F2, FRAP, XPD, CDKN, Ral DGS, IDT, CDH1, APC1, and ESR. The results showed that the methods disclosed herein are viable alternatives to the sodium bisulfite reaction. The studies herein utilized 2M magnesium bisulfite solution, which is diluted in the sample to about 1.3M. Use of a more concentrated magnesium bisulfite solution would yield higher bisulfite concentration for conversion, while still keeping reaction volumes to a minimum. Such increased bisulfite concentration in the reaction mixture could easily be employed, and would be expected to enhance PCR yields. The optimization of such reaction parameters, including volume and/or concentration of magnesium bisulfite solution, temperature, pH and other reaction conditions are expected to lead to more complete conversion, and are well within the skill of the art.

Evaluation of HPLC Model System

A model system using a synthetic, four base oligonucleotide, ATCG, was employed to determine the rate of cytosine to uracil conversion by HPLC. Samples contained Et4NOH, no additive, tetramethyl ammonium chloride (TMAC), or guanidine HCl in the magnesium bisulfite reaction. The composition of the samples of Examples 19-22 is shown in Table 5 below.

TABLE 5

Ex. 19

Ex. 20

Ex. 21

Ex. 22

ATCG 2.5 μL

ATCG 2.5 μL

ATCG 2.5 μL

ATCG 2.5 μL

2M Mg(HSO3)

2M Mg(HSO3)

2M Mg(HSO3)

2M Mg(HSO3)

16.3 μL

16.3 μL

16.3 μL

16.3 μL

(~1.3M final)

(~1.3M final)

(~1.3M final)

(~1.3M final)

20% Et4NOH 2

—

TMAC 1.25 μL

3M Guanidine HCl

μL

0.83 μL

(0.1M final)

Water 4.2 μL

Water 6 μL

Water 4.95 μL

Water 5.4uL

pH ~ 4

pH ~3

pH ~3

pH ~3-4

Each sample was heated at 50° for about 28 minutes. The pH of the samples was measured after heating with pH paper, and is therefore approximate. All samples reacted comparably to each other, with the Et4NOH reaction performing slightly better than the others.

Another HPLC study was conducted evaluating Et4NOH, NaOH, Et4NCl, and guanidine thiocyanide as catalysts. The composition of the samples (Examples 23-26) is shown in Table 6, below.

TABLE 6

Ex. 23

Ex. 24

Ex. 25

Ex. 26

ATCG 2.5

ATCG 2.5 μL

ATCG 2.5 μL

ATCG 2.5 μL

μL

2M Mg(HSO3)2

2M Mg(HSO3)2

2M Mg(HSO3)2

—

16.3 Ml

16.3 μL

16.3 μL

(~1.3M final)

(~1.3M final)

(~1.3M final)

20% Et4NOH 2

5M NaOH 0.5

2M Et4NCl 2 μL

2M guanidine

μL

μL

thiocyanide

16.3 μL

Water 4.2 μL

Water 5.7uL

Water 4.2 μL

Water 6.2 uL

pH ~3

pH ~3

pH ~2

pH ~4

Each sample was heated at 50° for about 32 minutes. pH was measured after heating with pH paper, and is therefore approximate. Each of the reactions compared favorably to each other, with the exception of the guanidine thiocyanide reaction, which did not react at all. The Et4NOH reaction provided the beast results, with the NaOH reaction being nearly as effective. The Et4NCl reaction was useable, but was less effective than either the NaOH reaction or the Et4NOH reaction. Thus, pH may be important in the reaction.

Applicants have also discovered that, although they see significant benefits in using magnesium bisulfite instead of sodium bisulfite, significant improvements may also be seen, regardless of which bisulfite is used, with the modified purification processes discussed herein. Processes for purification are further discussed in the application entitled “Improved Bisulfite Method” (U.S. application Ser. No. 60/498,996 filed Aug. 29, 2003, and also application Ser. No. 60/520,941 (5109P2) having the same title and filed Nov. 17, 2003), assigned to the Assignee hereof, and which is incorporated by reference in its entirety. One embodiment of that process uses a Microcon 100 (Millipore), or similar, size-exclusion device. According to one embodiment of that method, the sample and 200 μL of water was added to the Microcon 100 device, and the sample was then spun in the device at approximately 2800 RPM for about 8 minutes (as per manufacturers recommendation). The resultant filtrate was removed. Two subsequent washes with about 300 μL water, each spun at about 2800 RPM for 8 minutes followed. After each, the filtrate was again removed. About 300 μL 0.1N NaOH was added and spun at approximately 2800 RPM for about 8 minutes. Again, the filtrate was removed. After addition of about 300 μL of water, the sample was spun in the device at 2800 RPM for about 6-8 minutes. The filtrate was removed and about 50 μL TE buffer was added. After about 5 minutes before it was inverted to collect the purified DNA sample in a centrifuge. Approximately 60 μL were collected.

While the above-described methods of PCR and sequencing are currently preferred, they are not the only methods useable. The present invention is not limited to these any particular embodiments, or any of the examples above. Rather, other variants of these methods will be apparent to those skilled in the art and are within the scope and spirit of the invention disclosed herein.